Controlled Cytoplast Arrest and Morula Aggregation Enhance Development, Cryoresilience, andIn VivoSurvival of Cloned Sheep Embryos

生物 细胞质 胚泡 胚胎 男科 细胞生物学 克隆(编程) 重编程 遗传学 细胞 胚胎发生 计算机科学 医学 程序设计语言
作者
Zachariah L. McLean,Sarah Jane Appleby,Lisanne M Fermin,H. V. Henderson,Jingwei Wei,David N. Wells,Björn Oback
出处
期刊:Cellular Reprogramming [Mary Ann Liebert, Inc.]
卷期号:23 (1): 14-25 被引量:4
标识
DOI:10.1089/cell.2020.0078
摘要

Zona-free somatic cell transfer (SCT) and embryo aggregation increase throughput and efficiency of cloned embryo and offspring production, respectively, but both approaches have not been widely adopted. Cloning efficiency is further improved by cell cycle coordination between the interphase donor cell and metaphase-arrested recipient cytoplast. This commonly involves inclusion of caffeine and omission of calcium to maintain high mitotic cyclin-dependent kinase activity and low calcium levels, respectively, in the nonactivated cytoplast. The aim of our study was to integrate these various methodological improvements into a single work stream that increases sheep cloning success. We show that omitting calcium during zona-free SCT improved blastocyst development from 6% to 13%, while caffeine treatment reduced spontaneous oocyte activation from 17% to 8%. In a retrospective analysis, morula aggregation produced high morphological quality blastocysts with better in vivo survival to term than nonaggregated controls (15% vs. 9%), particularly after vitrification (14% vs. 0%). By combining cytoplast cell cycle control with zona-free embryo reconstruction and aggregation, this novel SCT protocol maximizes the benefits of vitrification by producing more cryoresilient blastocysts. The presented cloning methodology is relatively easy to operate and further increases throughput and efficiency of cloned embryo and offspring production. Integration of additional reprogramming steps or alternate donor cells is straightforward, providing a flexible workflow that can be adapted to changing experimental requirements.
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